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恶性卡他热病毒主要蛋白的鉴定与特性分析

Identification and characterization of the major proteins of malignant catarrhal fever virus.

作者信息

Li H, Shen D T, Davis W C, Knowles D P, Gorham J R, Crawford T B

机构信息

Animal Diseases Research Unit, USDA Agricultural Research Service, Pullman, WA.

出版信息

J Gen Virol. 1995 Jan;76 ( Pt 1):123-9. doi: 10.1099/0022-1317-76-1-123.

Abstract

Malignant catarrhal fever virus (MCFV), a gamma-herpesvirus, causes a severe inflammatory and lymphoproliferative disease of cattle and other susceptible ruminants. Polyclonal antisera and monoclonal antibodies (MAbs) to the Minnesota isolate of MCFV were produced and used to examine the characteristics of the viral proteins. Immunoprecipitation of antigens of the Minnesota isolate of MCFV with polyclonal antisera revealed at least 11 proteins with molecular masses ranging from 17 kDa to 145 kDa. Among 279 candidate anti-MCFV hybridomas, 14 were selected and clustered into six groups on the basis of the patterns of reactivity to viral proteins in immunoprecipitation and immunoblot. The group I MAbs exhibited strong neutralizing activity and recognized a glycosylation-dependent conformational epitope on a 110 kDa protein. The MAbs in group II bound a non-neutralizing conformational epitope on a 130 kDa non-glycosylated protein. A glycosylated protein complex of 115/110/105/78/45 kDa moieties was identified by the MAbs in group III. The MAbs in groups IV, V and VI reacted with non-glycosylated proteins of 36/34 kDa, 24 kDa and 17 kDa, respectively. Comparison of three MCFV isolates [the Minnesota isolate, the Austrian isolate (Au-732) and the African prototype isolate (WC-11)] revealed no apparent differences in immunoprecipitation patterns with the single exception that the 110 kDa protein of WC-11 was slightly smaller than its counterpart in the Minnesota isolate.

摘要

恶性卡他热病毒(MCFV)是一种γ-疱疹病毒,可引发牛及其他易感反刍动物严重的炎症和淋巴细胞增生性疾病。制备了针对MCFV明尼苏达分离株的多克隆抗血清和单克隆抗体(MAb),并用于研究病毒蛋白的特性。用多克隆抗血清对MCFV明尼苏达分离株的抗原进行免疫沉淀,结果显示至少有11种分子量在17 kDa至145 kDa之间的蛋白质。在279个候选抗MCFV杂交瘤中,挑选出14个,并根据免疫沉淀和免疫印迹中对病毒蛋白的反应模式将其分为六组。I组单克隆抗体表现出强中和活性,并识别110 kDa蛋白上一个依赖糖基化的构象表位。II组单克隆抗体结合130 kDa非糖基化蛋白上的一个非中和性构象表位。III组单克隆抗体鉴定出一个由115/110/105/78/45 kDa部分组成的糖基化蛋白复合物。IV、V和VI组单克隆抗体分别与36/34 kDa、24 kDa和17 kDa的非糖基化蛋白发生反应。对三种MCFV分离株[明尼苏达分离株、奥地利分离株(Au-732)和非洲原型分离株(WC-11)]进行比较,结果显示免疫沉淀模式没有明显差异,唯一的例外是WC-11的110 kDa蛋白略小于明尼苏达分离株中的对应蛋白。

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